Difference between revisions of "Team:U of Guelph/Experiments"

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<h1 class="exEntery">Confirmation of SDM Success</h1>
 
<h1 class="exEntery">Confirmation of SDM Success</h1>
<p class="descP">A double restriction enzyme digest was conducted to ensure that the PstI cut site had been added correctly. A single restriction enzyme digest and undigested plasmid were used as controls. All digestion products were run on an agarose gel and visualized using either Novel Juice (FroggaBio) or SyBr.  
+
<p class="descP">A double restriction enzyme digest was conducted to ensure that the PstI cut site had been added correctly. A single restriction enzyme digest and undigested plasmid were used as controls. All digestion products were run on an agarose gel and visualized using either Novel Juice (FroggaBio) or SyBr. Samples were frozen in a -20&#176;C freezer for further use.
 
</p>
 
</p>
  
 
<h1 class="exEntery">Isolation of pET-28a(PstI) from DH5a</h1>
 
<h1 class="exEntery">Isolation of pET-28a(PstI) from DH5a</h1>
<p class="descP"> Here include information on how we isolated and purrified pET-28a(PstI) from DH5a/pET-28a</p>
+
<p class="descP"> pET-28a was purified from DH5&alpha;/pET-28a cells using a miniprep kit (Thermofisher Scientific). Purified DNA concentration was checked using a nanodrop and samples were frozen in a -20&#176;C freezer for further use.</p>
  
<h1 class="exEntery">Addition of EcoRI and PstI to FRC and OXC</h1>
+
<h1 class="exEntery">Addition of EcoRI and PstI to <i>frc</i> and <i>oxc</i></h1>
<p class="descP"> Here include information on how we designed FRC and OXC, ordered them, designed primers and added the RE sites and how we checked that it had worked</p>
+
<p class="descP"> PCR was used to add EcoRI and PstI cut sites to the ends of <i>frc</i> and <i>oxc</i>. PCR primers and synthesized <i>frc</i> and <i>oxc</i> were all obtained from IDT.</p>
  
<h1 class="exEntery">Adding FRC and Oxc to pET-28a(PstI)</h1>
+
<h1 class="exEntery">Adding <i>frc</i> and <i>oxc</i> to pET-28a</h1>
<p class="descP"> Here include information on how we RE digested FRC, OXC and pET-28a and preformed two separate ligations.</p>
+
<p class="descP"> The genes <i>frc</i> and <i>oxc</i> were added individually to pET-28a using standard ligation techniques.
<h1 class="exEntery">Transformation of pET-28a(PstI)<i>frc</i> and pET-28a(PstI)<i>oxc</i> into DH5a</h1>
+
</p>
<p class="descP"> Here include information on how we transformed FRC and OXC into DH5a</p>
+
<h1 class="exEntery">Transformation of pET-28a<i>frc</i> and pET-28a<i>oxc</i> into DH5&alpha;</h1>
<h1 class="exEntery">Isolation of pET-28a(PstI)<i>frc</i> and pET-28a(PstI)<i>oxc</i> from DH5a</h1>
+
<p class="descP"> Using standard heat shock techniques pET-28a<i>frc</i> and pET-28a<i>oxc were transformed into DH5&alpha;.
<p class="descP"> Here include information on how we isolated and purrified pET-28a(PstI)<i>frc</i> and pET-28a(PstI)<i>oxc</i> from DH5a</p>
+
Transformed cells were incubated for 1 hour at 37&#176;C with rotation (using our homemade rotator) then plated on Kanamycin plates.</p>
<h1 class="exEntery">Confermation of the Presence of <i>frc</i> and <i>oxc</i></h1>
+
 
<p class="descP"> Here include information on how we confirmed the presence of <i>frc</i> and <i>oxc</i></p>
+
<h1 class="exEntery">Confirmation of the Presence of <i>frc</i> and <i>oxc</i></h1>
 +
<p class="descP"> Colony PCR was used to confirm the presence of <i>frc</i> and <i>oxc</i> from the colonies grown from the transformation. One of each type of colony was selected to make liquid culture, and then glycerol stocks from for long term storage of the transformed bacteria.</p>
  
 
<h1 class="descSub">Protocols</h1>
 
<h1 class="descSub">Protocols</h1>

Revision as of 18:05, 25 October 2017

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Experiments

Experiment Overview

Our experimental goal this year was to clone frc and oxc into E. coli DH5α using pET-28a. To accomplish this goal we had frc and oxc synthesized by IDT and used PCR to add the correct restriction enzyme sites. Site directed mutagenesis was used to add the PstI cut site to pET-28a, then frc and oxc were inserted using standard restriction enzyme digests and ligation. pET-28afrc and pET-28aoxc were then transformed into DH5α.

Preparation of Competent Cells

This year we prepared two different types of competent cells, DH5α and BL21. We used a chemical competency method involving calcium chloride. As the final step in preparation all cells were frozen in either 50 µl or 100 µl volumes by submersion in liquid nitrogen. Competent cells were then stored in a -80°C freezer for further use.

pET-28a isolation

pET-28a was purified from DH5α/pET-28a cells provided by Cezar Khursigara's Lab using a miniprep kit (Thermofisher Scientific). Purified DNA concentration was checked using a nanodrop and samples were frozen in a -20°C freezer for further use.

Site Directed Mutagenesis of pET-28a

PCR was used to conduct site directed mutagenesis to add a PstI cut site to pET-28a. Two basepairs were changed at the wild type XhoI cut site to change the sequence from ctcgag to ctgcag. Primers were ordered from IDT.

Confirmation of SDM Success

A double restriction enzyme digest was conducted to ensure that the PstI cut site had been added correctly. A single restriction enzyme digest and undigested plasmid were used as controls. All digestion products were run on an agarose gel and visualized using either Novel Juice (FroggaBio) or SyBr. Samples were frozen in a -20°C freezer for further use.

Isolation of pET-28a(PstI) from DH5a

pET-28a was purified from DH5α/pET-28a cells using a miniprep kit (Thermofisher Scientific). Purified DNA concentration was checked using a nanodrop and samples were frozen in a -20°C freezer for further use.

Addition of EcoRI and PstI to frc and oxc

PCR was used to add EcoRI and PstI cut sites to the ends of frc and oxc. PCR primers and synthesized frc and oxc were all obtained from IDT.

Adding frc and oxc to pET-28a

The genes frc and oxc were added individually to pET-28a using standard ligation techniques.

Transformation of pET-28afrc and pET-28aoxc into DH5α

Using standard heat shock techniques pET-28afrc and pET-28aoxc were transformed into DH5α. Transformed cells were incubated for 1 hour at 37°C with rotation (using our homemade rotator) then plated on Kanamycin plates.

Confirmation of the Presence of frc and oxc

Colony PCR was used to confirm the presence of frc and oxc from the colonies grown from the transformation. One of each type of colony was selected to make liquid culture, and then glycerol stocks from for long term storage of the transformed bacteria.

Protocols

Here we will include a detailed list of all the basic protocols used in our experiments. Specific parameters for things such as PCRs will be noted above

Competent Cells

Insert protocol here.

Plasmid Isolation

Insert protocol here.

Agarose Gel

Insert protocol here.

PCR

Insert protocol here.

PCR Purification

Insert protocol here.

Restriction Enzyme Digest

Insert protocol here.

Spread Plating

Insert protocol here.

Streak Plating

Insert protocol here.

Liquid Culture Inoculation

Insert protocol here.

Transformation

Insert protocol here.

Refrences

Note here we have to include references to places where we pulled our protocols including lab methods.

Rose, D. This is a test (2017). Sci. Awesome. 28-29

University of Guelph iGEM 2017